EP2472264B1 - Détection multiplex de cellules tumorales utilisant plusieurs agents se fixant à des marqueurs extracellulaires - Google Patents

Détection multiplex de cellules tumorales utilisant plusieurs agents se fixant à des marqueurs extracellulaires Download PDF

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EP2472264B1
EP2472264B1 EP12002007.8A EP12002007A EP2472264B1 EP 2472264 B1 EP2472264 B1 EP 2472264B1 EP 12002007 A EP12002007 A EP 12002007A EP 2472264 B1 EP2472264 B1 EP 2472264B1
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cells
cancer
markers
agents
epcam
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EP2472264A3 (fr
EP2472264A2 (fr
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Ola Winqvist
Magnus Thorn
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SentoClone International AB
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    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/53Immunoassay; Biospecific binding assay; Materials therefor
    • G01N33/574Immunoassay; Biospecific binding assay; Materials therefor for cancer
    • G01N33/57484Immunoassay; Biospecific binding assay; Materials therefor for cancer involving compounds serving as markers for tumor, cancer, neoplasia, e.g. cellular determinants, receptors, heat shock/stress proteins, A-protein, oligosaccharides, metabolites
    • G01N33/57492Immunoassay; Biospecific binding assay; Materials therefor for cancer involving compounds serving as markers for tumor, cancer, neoplasia, e.g. cellular determinants, receptors, heat shock/stress proteins, A-protein, oligosaccharides, metabolites involving compounds localized on the membrane of tumor or cancer cells
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/53Immunoassay; Biospecific binding assay; Materials therefor
    • G01N33/574Immunoassay; Biospecific binding assay; Materials therefor for cancer
    • G01N33/57407Specifically defined cancers
    • G01N33/57419Specifically defined cancers of colon

Definitions

  • the present invention relates to a method for detection of cancer cell or cancer cell elements in a biological sample, wherein the method comprises addition of a panel of agents which bind to three or more extracellular markers and wherein at least one agent is cancer specific.
  • the detection is carried out by a spectro-metric method.
  • the sentinel node concept first introduced by Raymond Cabanas (Cabanas et al., 1977), proposes that the lymphatic drainage from a primary tumour passes through one particular regional lymph node - the sentinel node - and then continues.
  • the sentinel node concept entails the possibility of multiple drainage pathways from different parts of the primary tumour, thus a patient can have more than one sentinel node.
  • the sentinel node is unique for each individual.
  • the tumour status of this node reflects the status of the regional lymphatic field and has a strong impact on prognosis, as reported in large follow-up studies of malignant melanoma and breast cancer.
  • sentinel node biopsy Due to the strong evidence of sentinel node status as a prognostic factor, sentinel node biopsy and eventual evaluation of presence or absence of metastatic tumour cells has become routine procedure for staging in many countries.
  • the diagnosis of the sentinel node also has impact on the treatment strategy selected once the sentinel node is diagnosed. If sentinel node status can be rapidly determined it can also provide valuable information for decision-making during surgery.
  • tumour cells For metastases ⁇ 0.05 mm and ⁇ 0.02 the probability of missing the presence of tumour cells was 69% and 75%, respectively. The method also relies upon the individual skill of the pathologist to detect tumour cells. A final common problem with the current method is shortage of personnel skilled in the art at hospital laboratories, which has implications on the availability and cost of these procedures.
  • RT-PCR reverse transcriptase polymerase chain reaction
  • flow-cytometric approaches Alternative methodologies of detection have also been reported, including reverse transcriptase polymerase chain reaction (RT-PCR) and flow-cytometric approaches.
  • RT-PCR methodology is more sensitive than the histopathological method, but it is also time consuming and the method has been found to produce false-positive results (Merrie et al., 1999; Noguchi et al., 1999).
  • mRNA is sensitive to degradation, a feature making handling and transport of the specimen difficult in a routine clinical setting.
  • Using intracellular markers like cytokeratin-20 or HMB-45 also requires an extra step in the antibody staining procedure.
  • Cells must be permeabilised with e.g. saponin before monoclonal antibodies can reach their targets adding at least 30 minutes to the procedure.
  • a flow cytometry based method is also known from WO 98/28622 A1 , wherein several markers are provided, including extracellular markers like CEA and CA15-3.
  • the present invention relates to a one step method for direct and simultaneous detection of a cancer cell or cancer cell element in a biological sample, namely tumour cell detection in sentinel nodes, metinel nodes, or other lymph nodes, the method comprising
  • the present invention relates to a method for detection of cancer cell or cancer cell elements in a biological example, wherein the method comprises addition of a panel of agents which bind to three or more extracellular markers and wherein at least one agent is cancer specific.
  • the detection is carried out by a spectrometric method.
  • the present invention thus encompasses a one step process by the use of a panel of agents which is added to said biological sample and thereby permitting direct simultaneous detection of several cancer specific markers, thus omitting the step of sentinel node dissection, staining of the dissection sample and the subsequent inspection by an experienced pathologist.
  • the present invention permits a considerably faster, robust, standardised analytical method based upon non-subjective physical characteristics with higher specificity, sensitivity and reproducibility.
  • tumour cell detection in sentinel nodes is a common procedure for cancer staging. Applying a panel of agents binding to extracellular markers that identify a certain tumour type allows for tumour cell detection with a very high sensitivity and specificity. A similar method can be applied for detection of cancer cells also in other tissues.
  • the present invention can be used for determining type of primary tumour in patients with metastases of unknown origin.
  • the method can provide valuable clues in the search for the primary tumour site.
  • the method can be used for monitoring of cell cultures for cell therapy against cancer (so called adoptive immunotherapy).
  • adoptive immunotherapy requires the need for detection of cancer cells in a single cell suspension
  • a panel of agents binding to extracellular markers identifying the cancer type that is being treated could be used in order to verify that the cancer cells are absent from the cell culture before administering cells back to the patient.
  • This application may also be used for the monitoring of patients during treatment and may be used as a tool to evaluate the effectiveness of a treatment regimen as well as a decisive tool for selection of appropriate therapy.
  • Usage of the present invention for tumour cell detection applications can be achieved by preparing a single cell suspension from different types of tissue.
  • the single cell suspension or a sample there from is incubated with a panel of fluorophore conjugated monoclonal antibodies binding to markers that identify the cancer type that should be detected.
  • the sample is analysed using flow cytometry and the results of the analysis are readily available.
  • the single cell suspension can be prepared from various sources, namely sentinel nodes, metinel nodes, or other lymph nodes.
  • a single cell suspension is prepared from either a lymph node draining the metastasis of unknown origin or from a biopsy of the metastasis.
  • several panels of fluorophore conjugated monoclonal antibodies can be used to identify specific primary tumour types that are frequently metastasised to the organ or tissue where the metastasis has been found.
  • the single cell suspension may need to be divided in several samples, all incubated with different panels of antibodies, in order to screen for the tumour type that has metastasised. Analysis using flow cytometry is possible also in this application of the present invention.
  • Verification of absence of tumour cells in cell cultures for cell therapy against cancer can be achieved using a similar method as detection of tumour cells in lymph nodes.
  • the single cell suspension is prepared from a sample of the cell culture. Using the same type of panel of monoclonal antibodies as for the application of tumour cell detection, the single cell suspension is incubated, washed and finally analysed using flow cytometry.
  • agents refers to all agents capable of binding or interacting with an extracellular marker, covering both already known agents, such as, e.g. commercially available monoclonal antibodies, and agents to be generated.
  • suitable agents are monoclonal antibodies, polyclonal antibodies, Fab fragments, (Fab') 2 fragments, Fv fragments, peptides, proteins, RNA molecules, polysaccharides, or any combination thereof.
  • panel of agents Is intended to mean a panel containing two or more agents, such as, e.g., three or more, four or more, five or more, six or more, seven or more, eight or more agents, nine or more, or ten or more agents-
  • the number of agents chosen may depend on the number of markers to be screened for and/or the capacity of the equipment used in the method for quantifying the number of individual cells, i.e. how many agents the equipment is capable of detecting simultaneously.
  • the number of cancer specific agents in the panel depends on the specific use, however, one or more cancer specific agents are present, such as, e.g., two or more, three or more, four or more, five or more, six or more, seven or more, eight or more agents, nine or more, or ten or more agents.
  • Preferably much more specific agents are employed such as e.g. at least 20, at least 30, at least 40, at least 50, at least 75 or at least 100 dependent on the availability of the cancer specific agents.
  • the cancer specific agents in a panel may all be specific for one type of cancer or may have specificities for different cancers types.
  • antibodies refers to all types of immunoglobulins, including IgG, IgM, IgA, IgD, IgE, and IgY.
  • the antibodies may be monoclonal or polygonal and may be of any species of origin, including (for example) mouse, rat, rabbit, horse, chicken, or human, or may be chimeric antibodies.
  • Polyclonal antibodies used to carry out the present invention may be produced by immunizing a suitable animal (e.g., rabbit, goat, etc.) with an antigen, collecting immune serum from the animal, and separating the polyclonal antibodies from the immune serum, in accordance with known procedures.
  • Monoclonal antibodies used to carry out the present invention may be produced in a hybridoma cell line according to known techniques.
  • Antibody fragments included within the scope of the present invention include, for example, Fab, F(ab') 2, and Fv fragments, and the corresponding fragments obtained from antibodies other than IgG. Such fragments can be produced by known techniques.
  • extracellular marker refers to markers expressed on the surface of cells.
  • tissue-specific extracellular marker refers to a marker that is expressed on the surface of a cell belonging to a certain type of tissue, e.g. tissue of epithelial or mesenchymal origin.
  • cancer-specific extracellular marker refers to a marker expressed on the surface of cancer cells
  • cancer-type specific extracellular marker refers to a marker expressed on the surface of a certain type of cancer cell, i.e. on the surface of a colon cancer cell, a breast cancer cell, etc.
  • cancer-subtype specific extracellular marker refers to a marker expressed on the surface of cancer cells, where the marker is indicative for a specific characteristic of the cancer cells, such as, e.g. aggressiveness, metastatic properties, invasiveness, capability of immunosuppression, chemotherapy sensitivity, and presence of tumour antigens relevant for Immunotherapy.
  • sentinel lymph node is intended to mean the first lymph node(s) to receive lymphatic drainage from a tumour.
  • metinel lymph node refers to the first lymph node(s) to receive lymphatic drainage from a metastasis.
  • true positives is intended to mean a test sample correctly tested positive.
  • true negatives is intended to mean a test sample correctly tested negative.
  • false negatives is intended to mean a test sample falsely tested negative.
  • Sensitivity True positives True positives + False positives
  • NPV negative predictive value
  • test By the term “reproducibility” is intended to mean the ability of a test to be independently reproduced with the same test results, such as, e.g., an inter- and intra-assay variability less than 10%.
  • labeling of agents is intended to mean conjugation of an agent to a molecule detectable by an instrument, such as, e.g., enzymes, fluorescent molecules, radioactive molecules, biotin, oligonucleotides, and/or polysaccharides.
  • cut-off value is intended to mean a value which is considered to be a value that gives a proper distinction between positive and negative patient cases (health status).
  • the panel of agents may be used for detecting cancer cells present in a human or animal body, such as, e.g. in the blood or in tissues.
  • the application relates to use of a panel of agents binding to extracellular markers, wherein at least one of the agents is cancer specific, for detecting disseminated cancer cells in tissues.
  • the panel of agents may be used for detecting cancer cells anywhere in the human or animal body, the use of the panel of agents will in the following be exemplified and described in further details for detecting cancer cells in the lymphatic system, without limiting the invention in any way to the specifically described.
  • the invention relates to a method for detecting a cancer cell or cancer cell element in a biological sample, the method comprising adding to said biological sample a panel of agents, which bind to three or more different extracellular markers, wherein at least one of the agents is cancer specific. Detection of cancer cells or cell elements is executed by a spectrometric method, namely flow cytometry.
  • lymph nodes In the histopathological and immunohistochemlcal methods used today for examination of lymph nodes, the lymph nodes are cut into thin frozen sections and stained. However, as only a small fraction of the lymph node is examined, micro-metastasis outside the sections chosen will inevitably not be detected. Also, even if tumour cells are present within the sections manual screening by histopathological and immunohistochemical methods frequently misses small metastases (s 0.10 mm) and individual cancer cells (Weaver et al.)
  • a single-cell suspension of cells from the sentinel or metinel node(s) Is prepared after the sentinel or metinel lymph node(s) are removed.
  • Samples of the single cell suspension are incubated with a panel of agents targeting extracellular markers and a high number of cells, such as, e.g. 100,000 cells or more are then analyzed by a method capable of quantifying the number and proportion of individual cells expressing specific extracellular markers.
  • a suspension of cells from the one or more sentinel or metinel lymph node(s) a randomized population of cells representative for the one or more whole lymph node(s) is provided.
  • analysis of a relatively high number of cells provides statistically secure evidence of absence of presence of tumour cells.
  • the cancer cells may be detected with a sensitivity of 90% or more, such as, e.g., 91% or more, 92% or more, 93% or more, 94% or more, 95% or more, 96% or more, 97% or more, 98% or more, 99% or more or 100%, meaning that 90% or more, such as, e.g., 91% or more, 92% or more, 93% or more, 94% or more, 95% or more, 96% or more, 97% or more, 98% or more, or 99% or more, or 100% of sentinel or metinel nodes containing cancer cells will be correctly diagnosed as positive.
  • 90% or more such as, e.g., 91% or more, 92% or more, 93% or more, 94% or more, 95% or more, 96% or more, 97% or more, 98% or more, or 99% or more, or 100% of sentinel or metinel nodes containing cancer cells will be correctly diagnosed as positive.
  • the advantage of higher sensitivity using the present invention is increasingly significant with decreasing size of metastases.
  • the probability of detecting a metastasis is only dependent upon the total number of tumour cells present in the lymph node.
  • the probability of detection has been shown to be dependent also upon the size of the metastasis.
  • the sensitivity of detection by anti-cytokeratln immunohistochemistry has been found to be only 53% for breast cancer sentinel nodes initially classified as negative by histopathotogical screening.
  • the risk of missing a metastasis was found to increase with decreasing size.
  • the probability of missing a metastasis ⁇ 0.10 mm was found to be 61%.
  • the probability of missing the presence of tumour cells was 69% and 75%, respectively (Weaver et al.).
  • Another advantage of the present invention is that by analysing several markers at a time, more detailed information about each sample is obtained, thus reducing the risk of false-positive results by taking into account individual variations in cell expression.
  • the method also does not rely upon detection of cytokeratin-20 which as described earlier is not a cancer-specific marker, which further reduces risk of a false-positive diagnosis.
  • the cancer cells may be detected with a specificity of 95% or more, such as, e.g., 96% or more, 97% or more, 98% or more, or 99% or more, or 100% meaning that 95% or more, such as, e.g., 96% or more, 97% or more, 98% or more, or 99% or more, or 100% of the sentinel or metinel lymph nodes being free of cancer cells will be correctly diagnosed as negative.
  • Another way to express the improved sensitivity and specificity of the present invention is by the negative predictive value, i.e. the probability of a sentinel or metinel node diagnosed as free of cancer cells to be correctly diagnosed, This value reflects the combined high sensitivity and specificity. While other known techniques currently used today are prioritizing specificity to sensitivity, the present invention allows for maintaining high levels of both sensitivity and specificity.
  • the present invention relates to a use, wherein the cancer cells may be detected with a negative predictive value of 90% or more, such as, e.g., 91% or more, 92% or more, 93% or more, 94% or more, 95% or more, 96% or more, 97% or more, 98% or more, or 99% or more, or 100% meaning that if a sample is identified as being negative for cancer cells by the method described herein, the probability of that sample actually being negative is 90% or more, such as, e.g., 91 % or more, 92% or more, 93% or more, 94% or more, 95% or more, 96% or more, 97% or more, 98% or more, or 99% or more, or even 100%.
  • a negative predictive value of 90% or more such as, e.g., 91% or more, 92% or more, 93% or more, 94% or more, 95% or more, 96% or more, 97% or more, 98% or more, or 99% or more, or even 100%.
  • a high negative predicted value is favourable in a method as described herein as the risk of the patient having removed any healthy tissue during surgery is greatly diminished.
  • the inter- and intra-assay variability is less than 10%, such as, e.g., less than 9%, less than 8%, less than 7%, less than 6%, less than 5%, less than 4%, less than 3%, less than 2%, or less than 1%.
  • the procedure may be standardised and executed by a broad range of processionals, such as, e.g., biomedical scientists and clinical laboratory scientists.
  • the currently used histopathological methods requires the presence of a skilled pathologist which also leads to a much more subjective evaluation of the samples as there may be up to 30-35% variability between the observations of two different pathologists.
  • Another advantage of the present invention is that the analysis of presence or absence of cancer cells in a human or animal sample may be performed in very short time. This is especially relevant if the method is used for intraoperative diagnosis of lymph node metastasis and micrometastasis, allowing the diagnosis to be provided during e.g. surgery of the primary tumour.
  • the cancer cells may be detected within 25 minutes or less, such as, e.g. within 20 minutes or less, within 15 minutes or less, within 10 minutes or less.
  • Staining of cells by using the intracellular marker cytokeratin-20 suffers from the drawback that the cells have to be permeabilised with saponin to allow the agents to enter the cells, thereby adding time to the procedure.
  • the average time for performing an analysis using cytokeratin-20 is about 45 minutes. Accordingly, by using agents binding to extracellular markers the time of the analysis is reduced significantly.
  • the first strategy is to look for markers that changes level of expression when the cell becomes cancerous. With support from data showing that a certain cancer type frequently expresses a certain marker while the normal cell originating from the same tissue does not, one is able to make the assumption that the cell is cancerous. In this case, the marker could be called "cancer specific” or "cancer-type specific”.
  • the second strategy is to look for ectopic cells, i.e. to look for markers that should normally not be expressed in the tissue where analysed cells were collected.
  • ectopic cells i.e. to look for markers that should normally not be expressed in the tissue where analysed cells were collected.
  • cancer cells originate from normal, "healthy”, cells and naturally many of the surface markers are shared between the normal cell and the cancerous cell.
  • cancer cells display an immature phenotype expressing developmental proteins, proteins that at early differentiation stages are shared between many cell lineage committed stem cells. The difference often lies in the level of expression of some of the markers.
  • the expression profile of a cancer cell is unique for each Individual and may even vary between cancer cells of the same origin.
  • the same marker can in some cases provide evidence that a cell expressing that marker is a cancer cell, and in other cases not To appoint a certain marker a "cancer marker" must thus be made with additional information, such as, what type of cancer should be detected, to what frequency a certain marker is expressed by a certain cancer type, and in what tissue the cell expressing the marker was found.
  • Detection of cancer cells should thus ideally take into account individual variations.
  • One certain marker may be expressed by many cells of a certain cancer type, but not all cells. Cancerous cells originating from a certain tissue may lose expression of a certain marker normally expressed by that tissue.
  • One setup wherein the panel described herein is very useful is for detection of spread of cancer, i.e. the presence of metastasis including micrometastasis in the lymphoid system, such as in the sentinel and/or metinel lymph nodes.
  • the panel for use in such a setup should preferably contain one or more agents binding to general tissue-specific extracellular markers, such as, e.g., epithelial and/or mesenchymal extracellular markers. Almost all cancer cells will express at least one of these markers as they are derived from either epithelial or mesenchymal cells. In contrary, most cells present in a healthy lymph node do not normally express such markers. Accordingly, by including at least one agent binding to a general epithelial and/or mesenchymal marker, it is ensured that any cell not normally present in the lymph node is detected. However, as some non-cancerous cells having tissue-specific extracellular markers may also be present in lymph nodes (for example naevus cells containing mesenchymal extracellular markers) it is important to include at least one cancer-specific agent in the panel.
  • general tissue-specific extracellular markers such as, e.g., epithelial and/or mesenchymal extracellular markers. Almost all cancer cells will express at
  • the panel must contain one or more agents binding to cancer-type specific extracellular markers, wherein the cancer-type specific marker is carbohydrate antigen 19-9 (CA19-9).
  • the cancer-type specific marker is carbohydrate antigen 19-9 (CA19-9).
  • CA19-9 carbohydrate antigen 19-9
  • any such agent can be used that is already identified or at present unknown.
  • Markers that can be used include specific extracellular markers, general epithelial markers, epithelial specific antigen, epidermal growth factor, mesenchymal extracellular markers, cancer-type specific markers, and cancer-subtype specific markers as well as markers for "solid tumours and other types of tumours", colon cancer cells, urinary bladder cancer cells, malignant melanoma cells, breast cancer cells, prostate cancer cells, ovarian cancer cells, lung cancer cells.
  • markers are BC-10, carbohydrate antigen 125 (CA125), carbohydrate antigen 15-3 (CA15-3), carbohydrate antigen 19-9 (CA19-9), carbohydrate antigen 242 (CA242), carcino embryonic antigen (CEA), Ep-CAM, G250, MDR1, MDR2, MSH-R, NY-ESO-1, PRL-R, PSMA, RCAS1, STN, TA-90, and Beta 2-microglobulin (B2M), wherein Ep-CAM and CA19-9 are obligatory.
  • CEA carcino embryonic antigen
  • Ep-CAM Ep-CAM
  • G250 MDR1, MDR2, MSH-R, NY-ESO-1
  • PRL-R PSMA
  • RCAS1 RCAS1
  • STN TA-90
  • Beta 2-microglobulin B2M
  • Agents that can be used include agents binding to tissue-specific extracellular markers, general epithelial markers, mesenchymal extracellular markers, cancer-type specific, and/or cancer-subtype specific extracellular markers and agents binding to cancer-type specific extracellular markers selected from markers for breast cancer, colon cancer, esophagus cancer, kidney cancer, liver cancer, lung cancer, malignant melanoma, ovary cancer, pancreas cancer, prostate cancer, rectum cancer, stomach cancer, thyroid cancer, or any combination thereof.
  • the possible agents include monoclonal antibodies or fragments thereof binding one or more of the markers characteristic for colon cancer, malignant melanoma cells, breast cancer cells, prostate cancer cells, ovarian cancer cells, lung cancer cells.
  • agents are monoclonal antibodies to carcino embryonic antigen (CEA), carbohydrate antigen 15-3 (CA15-3), carbohydrate antigen 125 (CA125), carbohydrate antigen 19-9 (CA19-9), carbohydrate antigen 242 (CA242), Ep-CAM, G250, RCAS1, STN, TA-90, BC-10, NY-ESO-1, MSH-R, PRL-R, and PSMA.
  • CEA carcino embryonic antigen
  • CA15-3 carbohydrate antigen 15-3
  • CA125 carbohydrate antigen 125
  • CA19-9 carbohydrate antigen 242
  • Ep-CAM Ep-CAM
  • G250 RCAS1
  • STN STN
  • TA-90 TA-90
  • BC-10 NY-ESO-1
  • MSH-R TA-90
  • PRL-R PRL-R
  • agents binding to markers characteristic for a specific subtype of cancer cells may also be included in the panel.
  • markers may be markers indicating the following characteristics of the tumour/tumour cells, namely e.g. aggressiveness, metastatic properties, invasiveness, capability of immunosuppression, chemotherapy sensitivity, and presence of tumour antigens relevant for immunotherapy.
  • the treatment of the cancer may be tailored based on the specific tumour subtype. It is for example known that there is a series of membrane proteins called Multi Drug Resistance (MDR) proteins which may be heavily expressed in cancer cells and are able to pump anticarcinogenic agents out of the cancer cell, leaving the cancer cells insensitive or less sensitive to anticarcinogenic substances.
  • MDR Multi Drug Resistance
  • cancer cells By including one or more markers binding to MDR it is possible to determine whether the cancer cells will be sensitive towards treatment with chemotherapeutics and if so, administer chemotherapeutics as part of the same treatment regimen. However, if cancer cells prove to be insensitive to chemotherapeutics, other treatment regimens can be set up immediately.
  • Another use of a panel as described herein is for identifying the origin of a cancer metastasis. I.e. a situation where one or more metastases are identified in a patient, however, the location of the primary tumour having metastasized is not known.
  • Theoretically primary tumours originate from the cells present in the organ or tissue in which the tumour develops.
  • a metastasis of a primary tumour is defined as a cancer resulting from the spread of a primary tumour.
  • the metastasis process depends on the cancer cells acquiring two separate abilities - increased motility and invasiveness. Cells that metastasize are basically of the same kind as those in the original tumour. If a cancer arises in e.g. the colon and metastasizes to e.g. the liver, the cancer cells in the liver are colon cancer cells. However, the cells have acquired increased motility and the ability to invade another organ.
  • a panel according to the invention containing one or more agents binding to cancer-type specific and/or cancer sub-type specific extracellular markers it may be possible to determine the origin of the metastasis, i.e. to determine in which tissue the primary tumour have developed.
  • the panel may further comprise one or more agents binding to tissue-specific extracellular markers, such as, e.g., general epithelial and/or mesenchymal extracellular markers.
  • tissue-specific extracellular markers such as, e.g., general epithelial and/or mesenchymal extracellular markers.
  • Metastasis may be found anywhere in the human or animal body, however, the most common sites to find a metastasis is in the lymph nodes, liver, lungs, skeleton, brain, ovaries, adrenal glands, and abdominal cavity.
  • the panel must contain one or more agents binding to cancer-type specific extracellular markers.
  • any such agent or marker can be used that is already identified or at present unknown.
  • any such agent or marker can be used that is already identified or at present unknown.
  • Markers that can be used include specific extracellular markers, general epithelial markers, epithelial specific antigen, epidermal growth factor, mesenchymal extracellular markers, and cancer-type specific markers as well as markers for colon cancer cells, urinary bladder cancer cells, malignant melanoma cells, breast cancer cells, prostate cancer cells, ovarian cancer cells, lung cancer cells.
  • markers are BC-10, carbohydrate antigen 125 (CA125), carbohydrate antigen 15-3 (CA15-3), carbohydrate antigen 19-9 (CA19-9), carbohydrate antigen 242 (CA242), carcino embryonic antigen (CEA), Ep-CAM, G250, MDR1, MDR2, MSH-R, NY-ESO-1, PRL-R, PSMA, RCAS1, STN, TA-90, and Beta 2-microglobulin (B2M). At least one of the agents binds to CA19-9 and at least one of the agents binds to EpCAM.
  • Agents that can be used include agents binding to tissue-specific extracellular markers, general epithelial markers, mesenchymal extracellular markers, cancer-type specific, and/or cancer-subtype specific extracellular markers as well as agents binding to cancer-type specific extracellular markers selected from markers for breast cancer, colon cancer, esophagus cancer, kidney cancer, liver cancer, lung cancer, malignant melanoma, ovary cancer, pancreas cancer, prostate cancer, rectum cancer, stomach cancer, thyroid cancer, or any combination thereof.
  • the possible agents include monoclonal antibodies or fragments thereof binding one or more of the markers characteristic for colon cancer, malignant melanoma cells, breast cancer cells, prostate cancer cells, ovarian cancer cells, and lung cancer cells.
  • agents Monoclonal antibodies to carcino embryonic antigen (CEA), carbohydrate antigen 15-3 (CA15-3), carbohydrate antigen 125 (CA125), carbohydrate antigen 19-9 (CA19-9), carbohydrate antigen 242 (CA242), Ep-CAM, G250, RCAS1, STN, TA-90, BC-10, NY-ESO-1, MSH-R, PRL-R, and PSMA.
  • CEA carcino embryonic antigen
  • CA15-3 carbohydrate antigen 15-3
  • CA125 carbohydrate antigen 125
  • carbohydrate antigen 19-9 CA19-9
  • carbohydrate antigen 242 CA242
  • Such labels may be from enzymes, fluorescent molecules, radioactive labels, biotin, and/or oligonucleotides.
  • the agents are labelled with fluorescent molecules such as, e.g. nucleic specific dyes, phycobiliproteins, cyanine derivatives, fluorescein derivatives, and rhodamine derivatives.
  • fluorescent molecules such as, e.g. nucleic specific dyes, phycobiliproteins, cyanine derivatives, fluorescein derivatives, and rhodamine derivatives.
  • the different agents used in the panel are preferably labelled with different labels, so they can be distinguished from one another.
  • the method may preferably be performed by a fluorescence measuring instrument, such as, e.g. a flow cytometer.
  • Sentinel lymph nodes from a patient with cancer indication are obtained by surgery. Briefly, the sentinel node is identified during surgery by peri-tumoral injections of a tracer substance, e.g. patent blue dye, which follows the lymphatic drainage and colours the first-draining lymph nodes blue.
  • a tracer substance e.g. patent blue dye
  • Single cell suspensions from the whole sentinel lymph node/s to be investigated are obtained by gentle pressure of the lymph nodes using a loose fit glass homogenizer in 5 ml PBS supplemented with 2% Fetal calf serum and 0.05% Sodium Azide (staining buffer) or in cell culture medium such as X-Vivo 15 or Aim 5.
  • Cell samples are then labelled in 100 ⁇ l staining buffer with a panel of fuorophore conjugated antibodies selected from tissue-specific, cancer-type specific and cancer-subtype specific extracellular markers and incubated at room temperature 15-30 minutes.
  • the sufficient amount of antibody used is determined by titration of each antibody using a positive control. Typically this amount is in the range of 0.1-0.5 ⁇ g.
  • samples are washed with 2 ml staining buffer and resuspended in 300 ⁇ l staining buffer before flow cytometric analysis.
  • the analysis is performed using instruments such as FACSAria, FACSCanto (Becton Dickinson) or Cytomics FC 500 (Beckman Coulter). Row cytometric analysis is performed collecting 100.000 events from each cell sample.
  • kits can be developed for numerous applications of the present invention.
  • Such kits could include all necessary agents, labels and fluids and instructions necessary to perform a certain test.
  • the kit could also include software to facilitate interpretation of the test results, with e.g. predefined cut-off rates between a positive and negative test result
  • a kit would include a panel of fluorescence labelled monoclonal antibodies, where the panel would be suitable for a certain type of test. Furthermore the kit would include fluids necessary to perform the test using flow cytometry and software capable of reliably interpreting the data generated from the analysis.
  • Background data may be obtained by performing tests on a large number samples with known status or known prevalence in the relevant population of the abnormality searched for.
  • Data generated by each test e.g. the proportion of events tested positive for each marker, will be collected along with information for categorisation of the population to which the test subject belongs, e.g. sex, age, disease, stage of disease, etc.
  • the data generated may be used for finding optimal cut-off values.
  • Cut-off values are needed as also true negative samples will show varying degrees of "positivity" due to biological (varying degrees of expression of markers also in normal state) and technical (background noise) reasons.
  • the cut-off value which maximises the area under the ROC curve should be chosen.
  • the clinical use of a test must be taken into account when deciding the cut-off value.
  • the cut-off value will be set accordingly, i.e. the cut-off values may be chosen with respect to the clinical use/purpose.
  • ROC curves cannot be used alone to decide the cut-off values, as the method does not take the prevalence of the abnormality searched for into account.
  • background data on the prevalence of the abnormality to be detected is needed.
  • the sensitivity and specificity of a test may vary with the prevalence of the condition searched for in the population to which the test subject belongs. Thus, it may be necessary to decide different cut-off values for different populations.
  • Reference intervals can be used for this purpose if the prevalence of the abnormality in different populations is known.
  • the reference interval is the estimated range of values that includes a certain percentage of the values among a relevant population. The most commonly used percentage is 95%.
  • Two reference intervals would have to be calculated for deciding of cut-off value, one interval for assumed negative samples and one interval for assumed positive samples.
  • the categorisation of each sample would be made based on the prevalence of the abnormality in the population from where the sample has been collected. The proportional size of each sample group should conform to the prevalence of the abnormality in the population. Based on the test results for each node, each sample would be categorised into an assumed negative group and a assumed positive group. Reference intervals can be generated for each group, and the cut-off value may be set to minimise the overlap from one reference interval to the other. The cut-off value may also be set to minimise the risk of e.g. a false negative diagnosis.
  • Reference intervals can be calculated two basic approaches. If the data generated conforms to a distributional function such as, e.g., the Normal distribution, the reference intervals can be calculated using a parametric method meaning that the distribution conforms to a mathematically defined statistical distribution, e.g. the Normal distribution. Using parametric methods is generally preferred since confidence intervals of reference intervals are generally narrower unless the sample size is very large.
  • a distributional function such as, e.g., the Normal distribution
  • the reference intervals can be calculated using a parametric method meaning that the distribution conforms to a mathematically defined statistical distribution, e.g. the Normal distribution.
  • Using parametric methods is generally preferred since confidence intervals of reference intervals are generally narrower unless the sample size is very large.
  • Prevalence of the abnormality to be detected may vary with e.g. age, sex, and disease/indication. Accordingly, access to large amounts of background data to determine reference intervals for each relevant population may further enhance the diagnostic performance when using the present invention for detection of tumour cells.
  • Comparing the data generated by an analysis with earlier data on true positive and true negative samples may optimise the cut-off rate between a positive and negative result, enabling even higher performance with respect to sensitivity, specificity and NPV.
  • interpretation of each test is performed by use of a software linked to a database with background data for each marker tested in relation to relevant populations.
  • the software may also be capable of generating data for use in the same database, which would allow for continuous fine-tuning of cut-off values for each test and relevant population.
  • the invention relates to a database storing results obtained by the flow cytometry method claimed herein and software for calculating and continuously refining cut-off values when the data material increases.
  • the database contains a plurality of data set, wherein each data set comprises data for a plurality of extracellular surface markers and corresponding type or types of cancer cells.
  • the invention relates to a method for identifying cancer cells as claimed herein further comprising a step of storing the obtained data set from the flow cytometry method (e.g. i) number of cells carrying an agent that binds to one or more extracellular markers, ii) type of cancer cells, iii) type of tissue and the like).
  • the step of storing the data may further comprise a step of inputting data of known origin with corresponding data set.
  • the present invention relates to a software program that when run on a computer is i) adapted to receive flow cytometry data set comprising data for extracellular markers, ii) adapted to compare the received data with data in a database, and iii) adapted to provide an output indicating a) the presence or absence of cancer cells, and optionally b) the type or types of cancer cells.
  • tumour marker CA19-9 known to be expressed on the surface of colon cancer cells. Analysis of the sample was best performed using the side scatter (SSC) for size and granularity and FL-1 reflecting the FITC conjugate stained cells. Cells double positive with regards to an increased SSC and a high fluorescence was identified as exemplified in Figure 1 . Even as low as 0.33% of added CCL221 cells was easily detected.
  • tumour cells were not present in the sample, Indicating a small fraction of false positive cells.
  • the experiment was performed using an antibody recognizing an EpCAM-like cell surface molecule expressed on colon cells adding from 0.0122-3% tumour cells to the PBL. Again, the tumour population was easily detected as a cluster of cells expressing high amount of the EpCAM-like protein and an increased SSC ( Figure 2 ). Even as few as 0.0122% cells were detected as a distinguished population of cells ( Figure 2 ). There was no problem in false positive cells using the EpCAM-like protein as a targeted cell surface marker since no events was recorded as double positive when no tumour cells were added.
  • Periheral blood leukocytes where obtained by Ficoli paque.
  • the colon cancer cell line CCL221 was grown as suggested by provider (ATCC).
  • a sentinel lymph node from a patient being diagnosed with colon cancer was obtained by surgery.
  • Single cell suspensions from the whole sentinel lymph node/s to be investigated were obtained by gentle pressure of the lymph nodes using a loose fit glass homogenizer.
  • CK20 cells were first washed in PBS supplemented with 2% BGS and 0.05% (w/v) Sodium Azide (staining buffer) and thereafter treated with Cytofix/Cytoperm (Becton Dickinson) according to the manufacturer's instructions. Thereafter the cells were retained in staining buffer supplemented with 0.3% saponin (w/v) (Sigma). Primary staining was performed with mouse anti-human CK20 antibody (Dakocytomation) or IgG2a isotype control (Dakocytomation) for 30 min.
  • Cells were washed and incubated for 30 min with a goat-anti-mouse antibody conjugated with allophycocyanine (APC) (Jackson Immunoresearch) or a donkey-anti-mouse antibody conjugated with fluorescein isothiocyanate (FITC) (Jackson Immunoresearch). Staining for cell surface markers was performed in staining buffer.
  • APC allophycocyanine
  • FITC fluorescein isothiocyanate
  • EpCAM epidermal cell adhesion marker
  • CA19-9 Anti-Carbohydrate Antigen 19-9
  • AF488 Alexa fluor 488
  • PerCP Peridinin-chlorophyll-protein complex
  • Isotype controls used were IgG2a (clone G155-178) conjugated with AF488 and IgG1 (clone MOPC-21) conjugated with PerCP, (Becton Dickinson).
  • Sentinel node no CK20 + (%) EpCAM + (%) CA19-9 + (%) EpCAM + CA19-9 + EpCAM + CA19-9 - EpCAM - CA19-9 + (%) 1 SN1 5.6 1.9 5.6 11 1 SN2 0.57 0.18 0.72 2.6 1 SN 3 0.17 0.051 0.093 0.41 2 SN1 0.69 1.3 0.42 2.5 2 SN2 0.13 0.15 0.13 1.0 3 SN 0.099 0.038 0.042 0.75 4 SN1 0.17 0.088 0.024 0.80 4 SN2 3.1 2.8 24.7 29 5 SN1 1.9 0.79 1.7 3.9 5 SN2 1.9 1.3 2.4 8.2 6 SN1 0.20 0.26 0.078 1.1 6 SN2 0.30 0.55 0.27 1.6 7 SN 1 0.18 0.069 1.3 1.4 7 SN2 0.18 0.064 0.65 0.76
  • the intra-assay variability for flow cytometric analysis of tumour surface markers was tested by splitting a sample into ten aliquots before flow cytometric analyses. From the dilution series samples with 0.037%, 0.11%, 0.33%, 1% and 3% added DLD-1 tumour cells and samples of PBMC alone were examined.
  • EpCAM and CA19-9 when presented separately, the number of positive events was determined in dot plots of respective fluorescence in log-scale versus linear SSC properties. Analysis of the total number of detected cells was performed by plotting log green fluorescence versus log red fluorescence and the events recorded as either EpCAM + CA19 - , EpCAM - CA19-9 + or EpCAM + CA19-9 + were accumulated. The resulting mean detection of colon cancer cells, standard deviation and coefficient of variation are listed in Table 2.
  • the mean values of tumour cells detected with EpCAM expression were close to those expected, indicating that almost all DLD-1 cells expressed EpCAM (Table 2).
  • the CV values obtained from the samples with 0.11, 0.33,1 and 3% added DLD-1 colon cancer cells were in the range of 4.6-10.7%, indicating very low intra-assay variability.
  • the mean number of detected cells for 0.037% added cells was 0.041 % (range 0.035-0.055%) and for PBMC with no addition of tumour cells 0.002 (range 0-0.004%) (Table 2).
  • CA19-9 expression was investigated the mean values of tumour cell recovery were lower than the expected numbers, again indicating that not all tumour cells express CA19-9 (Table 2).
  • the average background staining in PBMCs was 0.036%, which interferes with detection of tumour cells at low concentrations, but for 0.33, 1 and 3% added cells 67,71 and 82%, respectively, appear to express CA19-9.
  • the average CV for CA19-9 detection was 8.4%. Indicating low intra-assay variability.
  • the dynamic range from 0 to 3% cells was tested by performing regression analyses ( FIG. 12A-C ).
  • the sample coefficient of determination was 1 for EPCAM ( Fig. 12A ), CA19-9 + ( Fig, 12B ) and for double positive cells. ( Fig. 12C ), demonstrating a stable and reliable performance within the investigated range.
  • the correlation between observed numbers and expected number of tumour cells for EpCAM + ( Fig. 12A ) and for the sum of EpCAM + CA19-9 - , EpCAM - CA19-9 + and EpCAM + CA19-9 + cells ( Fig. 12C ) was close to what is expected from the theoretical number of added cells.
  • CA19-9 appears to be expressed on approximately 73% of DLD-1 tumour cells.
  • Sentinel lymph nodes from 7 patients were identified during surgery by peri-tumoral injections of a tracer substance.
  • Single cell suspensions from each lymph node were prepared using a loose-fit glass homogeniser. Staining for extracellular markers was performed in staining buffer. Cells were washed and incubated for 30 minutes with anti-EpCAM and and CA 19-9 conjugated with Alexa488 and PerCP, respectively.
  • Isotype controls were performed for each sentinel node stained, exemplified by the staining of of SN1 from patient 5 ( figure 8 A) .
  • Analysis was performed by acquiring 100.000 events from each sample using a FACSAria flow cytometer.
  • Pat no Sentinel node no: EpCAM + (% of total events) CA19-9 + (% of total events) 1 SN 1 1.9 5.6 1 SN 2 0.18 0.72 1 SN 3 0.051 0.093 2 SN 1 1.3 0.42 2 SN 2 0.15 0.13 3 SN 1 0.038 0.042 4 SN 1 0.088 0.024 4 SN 2 2.8 24.7 5 SN 1 0.79 1.7 5 SN 2 1.3 2.4 6 SN 1 0.26 0.078 6 SN 2 0.55 0.27 7 SN 1 0.069 1.3 7 SN 2 0.064 0.65
  • each sample would be categorised into a assumed negative group and a assumed positive group where the proportional size of each group would match the prevalence in the relevant patient population. Reference intervals would then be calculated for both groups.
  • the reference intervals can be calculated using a parametric method. Using parametric methods is generally preferred since confidence intervals of reference intervals is generally narrower unless the sample size is very large.
  • Comparing of the reference intervals for both groups of samples can be used to set an appropriate cut-off value.
  • the cut-off value could be set, e.g., to minimise the overlap of the intervals or to minimise the risk of a false-negative diagnosis.
  • the standard approach for detection of metastases in lymph nodes from colon cancer is immunohistochemical staining using CK20 antibodies.
  • intracellular staining of CK20 and detection with an APC-conjugated secondary antibody was performed.
  • CK20 positive cells have been described in PBMCs from healthy individuals, suggesting a normal transient existence of cytokeratin positive epithelial cells in the blood.
  • CK20 positive cells When we intracellularly stained PBMCs for CK20 we were able to detect 0.19% and 0.16% CK20 positive cells as exemplified in a colon cancer patient with metastatic disease and a healthy individual, respectively ( Fig. 9B , left panels). In contrast, 0.03% and 0.02% positivity was detected when an isotype control was used ( Fig. 9B , right panels).
  • Fig. 9B right panels
  • CK20 positive cells were identified at low levels even in healthy individuals and intracellular staining is more cumbersome, the usefulness of directly conjugated antibodies recognizing colon cancer cell surface makes was investigated.
  • the dilution series of DLD-1 supplemented tumour cells was therefore stained with antibodies specific for the two tumour-associated surface antigens EpCAM and CA19-9, conjugated with the fluorophores AF488 and PerCP, respectively.
  • the antigen CA19-9 is expressed on approximately 80% of the DLD-1 tumour cells ( Fig. 10B ).
  • the average ratio between CA19-9 + and the added number of cells for the 5 highest concentrations was 0.80 (range 0.73-0 91).
  • the background staining in PBMCs with no added colon cancer cells was slightly higher for CA19-9 than for EpCAM, with 0.017% cells being CA19-9 positive ( Fig. 10B . bottom panel), compared to 0.004% being EpCAM positive ( Fig. 10A , bottom panel).
  • the presence of tumour cells was readily detectable at as low concentrations as 0.11% added cells without interfering with background staining. So even though the background is slightly higher than that for staining with EpCAM, CA19-9 appears to be a useful marker for detection of colon cancer cells by flow cytometry.
  • SN1-3 In patient 1 three sentinel nodes were identified (SN1-3). In SN1 there was a clear presence of metastatic colon cancer cells, of which 5.6% were CK20 positive and the same fraction of cells were identified as being CA19-9 positive ( Fig. 13A ). EpCAM appeared to be expressed on a third (34%) of the metastatic cells (or 1.9% of total events). Metastatic cells were also present in SN2, 0.57% of the cells being CK20 positive and 0.72% being positive for CA19-9. EpCAM expression was 0.18%, which in comparison to the cytokeratin expression represents 32% of the metastatic cells, and 25% compared to the CA19-9 positive cells. However, the number of detected EpCAM positive cells are close to the Isotype control level. The investigation of SN3 revealed only very few events positive for CK20, EpCAM or CA19-9, close to the detection levels determined by isotype controls and thus SN3 was considered as being negative for the presence of metastatic colon cancer cells.

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Claims (5)

  1. Méthode à une étape pour la détection directe et simultanée d'une cellule cancéreuse ou d'un élément de cellule cancéreuse dans un échantillon biologique, à savoir la détection de cellules de tumeur dans des ganglions sentinelles, ganglions métinelles ou autres ganglions lymphatiques, la méthode comprenant
    i) ajouter audit échantillon biologique un panneau d'agents marqués qui se lient à trois ou plusieurs marqueurs extracellulaires différents, où au moins un des agents est spécifique au cancer et où le panneau continent :
    - un ou plusieurs agents se liant à des marqueurs extracellulaires spécifiques du type de cancer, où le marqueur spécifique du type de cancer est CA19-9, et
    - un ou plusieurs agents se liant à des marqueurs extracellulaires spécifiques au tissu qui sont des marqueurs extracellulaires épithéliaux généraux, où le marqueur épithélial général est Ep-CAM ;
    ii) soumettre l'échantillon biologique ainsi obtenu à une cytométrie en flux.
  2. Méthode selon la revendication 1, où les agents marqués se lient à quatre ou plus de marqueurs extracellulaires différents.
  3. Méthode selon la revendication 1 ou 2, où les agents sont des anticorps monoclonaux ou des fragments de ceux-ci.
  4. Méthode selon l'une quelconque des revendications précédentes, où les cellules cancéreuses sont détectées avec une sensibilité de 90% ou plus, comme par exemple 91% ou plus, 92% ou plus, 93% ou plus, 94% ou plus, 95% ou plus, 96% ou plus, 97% ou plus, 98% ou plus, 99% ou plus ou 100%.
  5. Méthode selon l'une quelconque des revendications précédentes, où les cellules cancéreuses sont détectées avec une spécificité de 95% ou plus, comme par exemple 96% ou plus, 97% ou plus, 98% ou plus, 99% ou plus ou 100% ce qui signifie que 95% ou plus, comme par exemple 96% ou plus, 97% ou plus, 98% ou plus, 99% ou plus ou 100% des ganglions lymphatiques sentinelles ou métinelles exemptes de cellules cancéreuses seront correctement diagnostiquées comme étant négatifs.
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EP2472264A3 (fr) 2012-10-17
RU2489720C2 (ru) 2013-08-10
US20110312511A1 (en) 2011-12-22
DK2472264T3 (en) 2016-02-29
JP5409395B2 (ja) 2014-02-05
CN101669031A (zh) 2010-03-10
JP2011503520A (ja) 2011-01-27
HUE028487T2 (en) 2016-12-28
WO2008104380A2 (fr) 2008-09-04
EP2472264A2 (fr) 2012-07-04
BRPI0807384A2 (pt) 2014-05-20
RU2009135780A (ru) 2011-04-10
SI2472264T1 (sl) 2016-06-30
EP2126579A2 (fr) 2009-12-02

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